Gebhardt Matthias, Mentlein Rolf, Schaudig Ulrich, Pufe Thomas, Recker Kristin, Nölle Bernhard, Al-Samir Kais, Geerling Gerd, Paulsen Friedrich P
Department of Anatomy, Christian Albrecht University of Kiel, Kiel, Germany.
Ophthalmology. 2005 Jun;112(6):1023-30. doi: 10.1016/j.ophtha.2005.01.023.
To study the distribution of isoforms of vascular endothelial growth factor (VEGF) and its receptors VEGFR1 and VEGFR2 in pterygia and to compare it with that in healthy conjunctivas.
Nonrandomized comparative (cadaver controlled) study with histopathologic correlations.
Tissue specimens from 75 patients treated for primary pterygia were analyzed using immunohistochemical studies as well as different molecular biological examinations. Healthy conjunctivas from 33 patients treated for cataracts as well as specimens from the conjunctiva, limbus, and lens of both eyes of 12 body donors served as controls.
Surgical specimens of pterygia and normal conjunctiva specimens were processed with paraffin, sectioned, stained using specific antibodies against VEGF and its receptors, and examined by light microscopy. The other part of both groups of specimens as well as specimens from body donors were prepared and analyzed by means of reverse-transcription polymerase chain reaction (RT-PCR), real-time RT-PCR, enzyme-linked immunosorbent assay, and Western blots.
Vascular endothelial growth factor and VEGFR1 and VEGFR2 were analyzed to indentify the splice variants of VEGF as well as the distribution and amount of VEGF and both receptors in pterygia and the control tissues.
In analysis of specimens from pterygium patients as well as normal conjunctivas, VEGF121 and VEGF165 were identified as the only VEGF splice forms expressed. In addition to VEGF, VEGFR1 and VEGFR2 were detected in pterygia and conjunctivas and immunostained within the epithelium of pterygia and conjunctivas and on intrapterygial and intraconjunctival endothelial cells. Levels of VEGFR1 and VEGFR2 mRNA were lower in pterygia than in conjunctivas but similar in limbal and pterygium samples. Vascular endothelial growth factor levels were higher in pterygia than in conjunctivas, but were similar in the limbus and pterygia.
The results reveal similar behaviors in limbal and pterygium epithelial cells in terms of VEGF and VEGFR expression, with the presumption that pterygia arise from limbal epithelial cells and that human conjunctivas are not a suitable control for the analysis of pterygia. Moreover, the results suggest that VEGF might play an active role in the physiology of conjunctival epithelial cells.
研究血管内皮生长因子(VEGF)及其受体VEGFR1和VEGFR2的亚型在翼状胬肉中的分布,并与健康结膜中的分布进行比较。
非随机对照(尸体对照)研究,并进行组织病理学相关性分析。
对75例接受原发性翼状胬肉治疗的患者的组织标本进行免疫组织化学研究以及不同的分子生物学检测分析。33例接受白内障治疗的患者的健康结膜以及12例尸体捐献者双眼的结膜、角膜缘和晶状体标本作为对照。
翼状胬肉手术标本和正常结膜标本用石蜡处理、切片,使用抗VEGF及其受体的特异性抗体染色,然后进行光学显微镜检查。两组标本的另一部分以及尸体捐献者的标本通过逆转录聚合酶链反应(RT-PCR)、实时RT-PCR、酶联免疫吸附测定和蛋白质免疫印迹法制备并分析。
分析血管内皮生长因子、VEGFR1和VEGFR2,以确定VEGF的剪接变体以及VEGF和两种受体在翼状胬肉和对照组织中的分布及含量。
在对翼状胬肉患者标本以及正常结膜的分析中,VEGF121和VEGF165被确定为仅表达的VEGF剪接形式。除VEGF外,在翼状胬肉和结膜中检测到VEGFR1和VEGFR2,并在翼状胬肉和结膜上皮内以及翼状胬肉内和结膜内的内皮细胞上进行免疫染色。翼状胬肉中VEGFR1和VEGFR2 mRNA水平低于结膜,但角膜缘和翼状胬肉样本中的水平相似。血管内皮生长因子水平在翼状胬肉中高于结膜,但在角膜缘和翼状胬肉中相似。
结果显示,在VEGF和VEGFR表达方面,角膜缘和翼状胬肉上皮细胞表现相似,据此推测翼状胬肉起源于角膜缘上皮细胞,并且人结膜不是分析翼状胬肉的合适对照。此外,结果表明VEGF可能在结膜上皮细胞的生理过程中发挥积极作用。
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